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首页> 外文期刊>Nucleic acids research >Influence of molecular weight of DNA on the determination of anti-DNA antibodies in systemic lupus erythematosus (SLE) sera by radioimmunoassay
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Influence of molecular weight of DNA on the determination of anti-DNA antibodies in systemic lupus erythematosus (SLE) sera by radioimmunoassay

机译:DNA分子量对放射免疫法测定系统性红斑狼疮(SLE)血清中抗DNA抗体的影响

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Using a radioimmuno assay (RIA) based on the Farr technique with radioactively labeled 3H-DNA for quantitative measurements of anti-DNA antibodies in sera of patients with systemic lupus erythematosus (SLE), the influence of molecular weight of DNA (ranging from 0.1 × 106 to 22.0 × 106 daltons) on binding and precipitation in this system has been investigated. Comparing our results with mathematical models it follows that one antibody molecule is fixed on the average to a statistical DNA segment of 2 × 106 to 4 × 106 daltons. Furthermore binding capacity of the DNA was found to be independent of the molecular weight, as demonstrated in a double label experiment using 14C and 3H-labeled DNA of different size. However, the amount of radioactivity precipitated was found to depend on the molecular weight of the labeled DNA following a non-linear function. It was calculated that a minimal ratio of fixed antibody molecules per a certain size of DNA was necessary for precipitation. The mathematical treatment of the observed non-linear precipitation dependence will be discussed using various statistical models. Our results indicate that the quantitative measurements of anti-DNA antibodies with the Farr technique e.g. for diagnosis and control of SLE in clinical immunology is highly dependent on the molecular weight of the labeled DNA used in the assay system and reliable results are only obtained with DNA of a sufficiently high molecular weight.
机译:使用基于Farr技术的放射免疫测定(RIA)和放射性标记的 3 H-DNA定量测定系统性红斑狼疮(SLE)患者血清中的抗DNA抗体,研究了该系统中DNA结合和沉淀的重量(从0.1×10 6 到22.0×10 6 道尔顿)。将我们的结果与数学模型进行比较,可以得出结论:一个抗体分子平均固定在2×10 6 至4×10 6 道尔顿的统计DNA片段上。此外,发现DNA的结合能力与分子量无关,如使用 14 C和 3 H标记的不同大小的DNA进行的双标记实验所证明的。然而,发现放射性的沉淀量取决于遵循非线性功能的标记DNA的分子量。经计算,每沉淀一定大小的DNA固定抗体分子的最小比例对于沉淀是必需的。将使用各种统计模型讨论观测到的非线性降水依赖性的数学处理。我们的结果表明,用Farr技术,例如,抗DNA抗体的定量测量。在临床免疫学中用于SLE的诊断和控制的方法高度依赖于测定系统中使用的标记DNA的分子量,只有使用足够高分子量的DNA才能获得可靠的结果。

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